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通过分子杂交检测实验感染小鼠中的肠道病毒RNA:亚基因组探针在定量斑点印迹和原位杂交中的特异性

Detection of enterovirus RNA in experimentally infected mice by molecular hybridisation: specificity of subgenomic probes in quantitative slot blot and in situ hybridisation.

作者信息

Zhang H Y, Yousef G E, Bowles N E, Archard L C, Mann G F, Mowbray J F

机构信息

Department of Experimental Pathology, St. Mary's Hospital Medical School, London, England.

出版信息

J Med Virol. 1988 Dec;26(4):375-86. doi: 10.1002/jmv.1890260405.

Abstract

Subgenomic cDNA clones representing defined regions of the genome of Coxsackie B3 virus were used as hybridisation probes to detect RNA of various enteroviruses in cell culture and mouse model systems. Radiolabelled probes were used in slot blots to quantitate the RNA in samples; biotinylated probes were used to localise virus RNA at the cellular level by in situ hybridisation with monolayers of infected cells or thin sections of tissue samples. Probes derived from the 5' or 3' terminal regions of Coxsackie virus RNA, which are highly conserved in the genus Enterovirus, detected RNA of various serotypes in infected cell cultures, but failed to hybridise with hepatitis A virus (HAV) RNA. Although HAV is clearly a Picornavirus, our data support the view that its taxonomic position within the enteroviruses should be reconsidered. The biotinylated probes were also used to detect in situ virus RNA in paraffin-embedded tissue samples from experimental mouse models of Coxsackie B3 virus-induced myocarditis or Coxsackie B1 virus-induced myositis. Since the integrity of the tissues was preserved during the process, and viral RNA was localised in the affected muscle fibres, this has enabled us unequivocally to relate the infecting virus to the underlying tissue injury.

摘要

代表柯萨奇B3病毒基因组特定区域的亚基因组cDNA克隆被用作杂交探针,以检测细胞培养和小鼠模型系统中各种肠道病毒的RNA。放射性标记的探针用于狭缝印迹法对样品中的RNA进行定量;生物素化的探针通过与感染细胞单层或组织样品薄片进行原位杂交,在细胞水平上定位病毒RNA。源自柯萨奇病毒RNA 5'或3'末端区域的探针在肠道病毒属中高度保守,可检测感染细胞培养物中各种血清型的RNA,但未能与甲型肝炎病毒(HAV)RNA杂交。尽管甲型肝炎病毒显然是一种小RNA病毒,但我们的数据支持这样一种观点,即应重新考虑其在肠道病毒中的分类地位。生物素化的探针还用于检测来自柯萨奇B3病毒诱导的心肌炎或柯萨奇B1病毒诱导的肌炎实验小鼠模型的石蜡包埋组织样品中的原位病毒RNA。由于在该过程中组织的完整性得以保留,并且病毒RNA定位于受影响的肌纤维中,这使我们能够明确地将感染病毒与潜在的组织损伤联系起来。

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